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The level of BLyS (BAFF) correlates with the titre of autoantibodies in human Sjögren’s syndrome
  1. X Mariette1,
  2. S Roux1,
  3. J Zhang2,
  4. D Bengoufa3,
  5. F Lavie1,
  6. T Zhou4,
  7. R Kimberly4
  1. 1Service de Rhumatologie, Hôpital de Bicêtre (Assistance publique-Hôpitaux de Paris (AP-HP)), Université Paris XI, INSERM EMI 0109, 94275 Le Kremlin Bicêtre, France
  2. 2Human Genome Sciences, Rockville, MD, USA
  3. 3Laboratoire d’Immunologie, Hôpital Saint-Louis (AP-HP), Université Paris VII, Paris, France
  4. 4Division of Clinical Immunology and Rheumatology, University of Alabama at Birmingham, Birmingham, AL, USA
  1. Correspondence to:
    Professor X Mariette, Service de Rhumatologie, Hôpital de Bicêtre, 78 rue du Général Leclerc, 94275 Le Kremlin, Bicêtre CEDEX, France;
    xavier.mariette{at}bct.ap-hop-paris.fr

Abstract

Background: Increased levels of B lymphocyte stimulator (BLyS) have been detected in serum from patients with systemic lupus erythematosus and rheumatoid arthritis.

Objective: To determine the level of BLyS in serum from patients with primary’s Sjögren’s syndrome (SS), another autoimmune disease in which B cell activation is high.

Methods: Serum samples from 49 patients with primary SS according to the revised European criteria were assayed for BLyS, quantitative immunoglobulins, and autoantibody levels and compared with samples from 47 healthy control subjects.

Results: The median level of BLyS was 5.99 ng/ml (25th-75th centile range 3.20–8.93 ng/ml) in SS v 2.49 ng/ml (25th-75th centile range 1.96–2.96 ng/ml) in healthy controls (p<0.001). More importantly, among patients with SS, the presence of anti-SSA antibodies was associated with significantly higher levels of BLyS (medians 7.90 ng/ml v 3.70 ng/ml; p=0.008) as was the presence of anti-SSB antibodies (medians 7.14 ng/ml v 3.70 ng/ml; p=0.02) and of rheumatoid factor (medians 7.70 ng/ml v 3.80 ng/ml; p=0.016). The level of BLyS in three patients with a monoclonal gammopathy was higher than in the other patients (medians 26.53 ng/ml v 5.92 ng/ml; p=0.13). Higher levels of BLyS were associated with higher levels of gammaglobulins and IgG. There was a strong correlation between BLyS and rheumatoid factor level (r=0.71, p<0.0001), anti-SSA IgG level (r=0.32, p=0.02) and anti-SSA IgM level (r=0.39, p=0.006).

Conclusion: In human SS the level of BLyS correlates with the level of autoantibodies. Thus, BLyS may play a part in activating specific autoreactive B cells and modulating the level of production of autoantibodies which are the hallmark of the disease. These findings raise the possibility of a novel therapeutic approach in human SS.

  • B lymphocyte stimulator
  • autoantibodies
  • Sjögren’s syndrome
  • BLyS, B lymphocyte stimulator
  • BSA, bovine serum albumin
  • ELISA, enzyme linked immunosorbent assay
  • HRP, horseradish peroxidase
  • PBS, phosphate buffered saline
  • RA, rheumatoid arthritis
  • SLE, systemic lupus erythematosus
  • SS, Sjögren’s syndrome
  • TNF, tumour necrosis factor

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A ctivation of autoreactive B cells is a common feature of various autoimmune diseases. Recent studies in animal models have emphasised the possible pathogenic role of B cells and autoantibodies in autoimmune diseases.1–3 The recent recognition of several members of the tumour necrosis factor (TNF) receptor superfamily, BCMA, TACI, and BAFF-R (BR3), on lymphocytes has provided important insight into B cell growth and survival.4–8 B lymphocyte stimulator (BLyS) (also named BAFF or TALL-1) appears to have an important role in autoimmunity because BLyS transgenic mice develop proteinuria and lupus-like disease,9,10 and a raised level of BLyS has been found in MRL-lpr/lpr and NZB/W-F1 autoimmune mice.11

The first two studies exploring this system in human autoimmune diseases showed raised levels of BLyS in serum from patients with systemic lupus erythematosus (SLE) and rheumatoid arthritis (RA).12,13 However, primary Sjögren’s syndrome (SS) is the autoimmune disease within which abnormal B cell activity is the most predominant. Very recently, Groom et al demonstrated that with increasing age BLyS transgenic mice develop severe sialadenitis and decreased saliva production. Moreover, they found raised levels of circulating BLyS in serum of humans with SS.14 We have assessed BLyS levels in serum from patients with primary SS and shown a correlation between the level of BLyS and both the level of immunoglobulins and the titre of autoantibodies.

SUBJECTS AND METHODS

Subjects

We studied consecutive patients seen during a six month period in the sicca syndrome and Sjögren’s syndrome consultation unit of Bicêtre Hospital in France. Forty nine patients fulfilled the diagnosis of primary SS according to the revised European criteria (4/6 of the EU diagnostic criteria, including at least one of anti-SSA and/or SSB antibodies, or a positive labial gland biopsy with a focus score ⩾1).15,16 None of these patients fulfilled criteria for another connective tissue disease. Control subjects (n=47) were healthy volunteer donors recruited from the blood bank at the University of Alabama at Birmingham.

Serological studies

After obtaining written informed consent, venous blood was collected by venepuncture. Total gammaglobulin level was determined by standard serum protein electrophoresis. IgG, IgA, and IgM levels were measured by nephelometry. Rheumatoid factor was also determined by nephelometry, while antinuclear antibodies were measured by indirect immunofluorescence. Anti-SSB antibodies were determined by antigen-specific enzyme linked immunosorbent assay (ELISA; ANA profile, Pharmacia-Upjohn, Freiburg, Germany). Anti-SSA IgG were determined by quantitative antigen-specific ELISA according to the manufacturer’s instructions (VARELISA SSA/Ro, Pharmacia-Upjohn). The same ELISA immunoassay was used for detection and quantification of anti-SSA IgM using an antihuman IgM horseradish peroxidase (HRP) conjugate. Immunofixation was performed to detect a monoclonal component in serum immunoglobulins.

A sandwich ELISA for measurement of the soluble form of BLyS™ was performed with modifications to previously described procedures.12 Briefly, 96 well plates were coated with purified murine anti-BLyS monoclonal antibody (clone 3D4, mIgG1) at 2 μg/ml in phosphate buffered saline (PBS) at 4°C overnight and blocked with 1% bovine serum albumin (BSA)/PBS. All specimens were diluted 1:10 in 3% BSA/PBS and incubated in the ELISA plate at 37°C for four hours. After washing, the plate was incubated first with 0.2 μg/ml biotin conjugated polyclonal anti-BLyS antibody and then with 1:30 000 diluted HRP conjugated streptavidin (Southern Biotechnology, Birmingham, AL). To avoid any confounding effect of rheumatoid factor activity, an mIgG1 isotype was used as a background control for the capture antibody with each specimen. The reaction was developed with trimethylbenzidine substrate (Sigma, St Louis, MO) and read in an E-Max plate reader (Molecular Devices, Sunnyvale, CA). In this assay, the absorbance values in the mIgG1 control wells were subtracted from the corresponding anti-BLyS capture wells and were typically <10% of total absorbance. There was no difference in values obtained with parallel serum and plasma samples. A standard curve using serial dilutions of recombinant BLyS was incorporated into each assay.

Statistical analysis

Statistical analysis were performed using Statview software (Abacus Concept Inc, Cary, NC, USA). Autoantibody, immunoglobulin, and BLyS levels were not normally distributed in patients with SS. Therefore, the non-parametric Mann-Whitney test was used to compare assay values in patients with those in controls. For correlations between the level of BLyS and the level of immunoglobulins and of autoantibodies, absolute values were log transformed to obtain a normal distribution and then Pearson’s correlation coefficient was calculated. All tests of significance were two tailed.

RESULTS

Forty nine patients with clinical SS met the revised European criteria for the classification of SS. Among these patients anti-SSA antibodies, anti-SSB antibodies, and rheumatoid factor were present in 31 (63%), 16 (33%), and 27 (55%) of the group, respectively. Three patients had a serum monoclonal component without any clinical evidence of lymphoma.

The mean (SD) levels of total gammaglobulins and of the individual IgM, IgG, and IgA classes were 14.0 (9.2) g/l, 1.6 (1.7) g/l, 15.6 (8.9) g/l, and 3.2 (1.8) g/l, respectively. As shown in fig 1A the median level of BLyS was 5.99 ng/ml (25th-75th centile range 3.20–8.93 ng/ml) in SS compared with 2.49 ng/ml (25th-75th centile range 1.96–2.96 ng/ml) in healthy controls (p<0.001). More importantly, among patients with SS, the presence of anti-SSA antibodies was associated with significantly higher levels of BLyS (medians 7.90 ng/ml v 3.70 ng/ml; p=0.008) as was the presence both of anti-SSB antibodies (7.14 ng/ml v 3.70 ng/ml; (p=0.02) (fig 1B) and of rheumatoid factor (7.70 ng/ml v 3.80 ng/ml; p=0.016) (fig 1C). The level of BLyS in the three patients with a monoclonal gammopathy was higher than in the other patients (26.53 ng/ml v 5.92 ng/ml; p=0.13).

Figure 1

BLyS levels in patients with SS. (A) Serum levels of BLyS in the patients with SS (n=49) were significantly higher than in normal donors (n=47), p<0.001. (B and C) Among patients with SS, BLyS levels were higher in patients with anti-SSA antibodies, anti-SSB antibodies, and in patients with RF (p=0.008, p=0.02, and p=0.016, respectively; Mann-Whitney test). The medians of each group were: normal, 2.49 ng/ml; SS, 5.99 ng/ml; SS with anti-SSA, 7.90 ng/ml; SS with anti-SSB, 7.14 ng/ml; SS without anti-SSA/SSB, 3.70 ng/ml; SS with RF, 7.70 ng/ml; SS without RF, 3.80 ng/ml.

Analysis of the 46 patients without a monoclonal gammopathy showed that higher levels of BLyS were associated with higher levels of gammaglobulins and IgG (fig 2). Interestingly, there was a strong correlation between BLyS and anti-SSA IgG level (r=0.32, p=0.02), anti-SSA IgM level (r=0.39, p=0.006), and rheumatoid factor level (r=0.71, p<0.0001) (fig 3).

Figure 2

Correlation between BLyS and immunoglobulins. Correlations between serum levels of BLyS and serum gammaglobulin (A), and IgG (B) were determined for the 46 patients with SS without a monoclonal component. Analysis was based on log10 transformed values. The correlation coefficient was determined by the Pearson product statistic and the regression line is represented by the solid line.

Figure 3

Correlation between BLyS and autoantibodies. Correlations between serum levels of BLyS and anti-SSA IgG (A), anti-SSA IgM (B) and serum RF (C) were determined by log10 transformed values. The correlation coefficient was determined by the Pearson product statistic and the regression line is represented by the solid line.

DISCUSSION

We have shown that the BLyS level is raised in the serum of patients with SS and is at least as high as in patients with RA and SLE. As in the two latter diseases, but contrary to the findings of Groom et al, BLyS levels correlated with the presence of autoantibodies, including anti-SSA/SSB and rheumatoid factor.14 This observation parallels data in BLyS transgenic mice, in which increases of autoantibody titres are out of proportion to increases in total serum immunoglobulin levels. The level of BLyS in our study also correlated with the titre of anti-SSA antibodies and rheumatoid factor, suggesting a role, either primary or secondary, for BLyS in modulating the level of autoantibody production. The inability of Groom and colleagues to detect these relationships in their patient collection compared with our cohort is, perhaps, not surprising. Firstly, there is an apparent difference in the relative sensitivities of the BLyS ELISAs in the two studies. For example, using different capture and detection antibodies, Groom did not detect any significant differences in BLyS level between controls and patients with RA and SLE. Indeed, with the reagents in our assay, such a difference has been demonstrated in several independent cohorts.12,13 Secondly, because only four patients with primary SS were Ro (SSA) negative, the power to detect differences in BLyS levels between Ro(SSA) positive and negative patients might have been insufficient.

In some autoimmune diseases, such as scleroderma and spondyloarthropathies, in which B cell activation is not predominant, raised levels of circulating BLyS have not been found.13 Most likely, the primary location for the production and normal physiological action of BLyS is in local lymphoid and inflammatory microenvironments, analogous to TNFα and other immune system cytokines. It is striking, therefore, that when B cell activity is persistently abnormal, raised circulating BLyS levels are apparent. In mice transgenic for BLyS, there is an expansion of marginal zone B cells,9–11 which are also overexpressed in salivary glands of patients with SS.14 In primary SS, with its predominant B cell activation, this expansion of MZ B cells is particularly evident. Whether the corresponding increase in B cells frequently displaying a rheumatoid factor activity,17 in monoclonal gammopathies, and in lymphomas arising in salivary glands or in other mucosal associated lymphoid tissues is related to persistent and high levels of BLyS mediated B cell stimulation remains unclear. Answers to this question will require careful longitudinal studies of several different patient groups with and without these characteristics. Such studies might also include phenotyping of B cells for expression of the three BLyS receptors, BCMA, TACI and BAFF-R (BR3), because the net effect of BLyS on B cell biology might be dependent of the type of receptor expressed by the target B cells.8

In any case, it is clear from animal models that the ability to antagonise BLyS has a major impact on the manifestations of autoimmune disease.7,18 Analogous to anti-TNF strategies, which now have widespread application in the clinic, both monoclonal antibodies and receptor fusion proteins are effective in vitro. The success of fusion proteins in vivo in blocking BLyS and ameliorating several autoimmune disease models raises the possibility of a novel therapeutic approach in human SS and other diseases in which BLyS may participate in activating specific autoreactive B cells and modulating the level of production of autoantibodies, which are the hallmark of the disease. The prospect of a new therapeutic strategy with mechanistic specificity, without widespread side effects, and with application to the more common human autoimmune diseases is very promising.

Acknowledgments

Grant support: Reagents provided by Human Genome Sciences, Inc.

BLyS™ is a trademark of Human Genome Sciences, Inc.

REFERENCES